AU681130B2 - Protein rib, a cell surface protein that confers immunity tomany strains of the group B streptococcus; process for purification of the protein, reagent kit and pharmaceutical composition - Google Patents
Protein rib, a cell surface protein that confers immunity tomany strains of the group B streptococcus; process for purification of the protein, reagent kit and pharmaceutical composition Download PDFInfo
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- AU681130B2 AU681130B2 AU63891/94A AU6389194A AU681130B2 AU 681130 B2 AU681130 B2 AU 681130B2 AU 63891/94 A AU63891/94 A AU 63891/94A AU 6389194 A AU6389194 A AU 6389194A AU 681130 B2 AU681130 B2 AU 681130B2
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Links
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Classifications
-
- C—CHEMISTRY; METALLURGY
- C07—ORGANIC CHEMISTRY
- C07K—PEPTIDES
- C07K14/00—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof
- C07K14/195—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria
- C07K14/315—Peptides having more than 20 amino acids; Gastrins; Somatostatins; Melanotropins; Derivatives thereof from bacteria from Streptococcus (G), e.g. Enterococci
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
- A61K39/02—Bacterial antigens
- A61K39/09—Lactobacillales, e.g. aerococcus, enterococcus, lactobacillus, lactococcus, streptococcus
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P31/00—Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
- A61P31/04—Antibacterial agents
-
- G—PHYSICS
- G01—MEASURING; TESTING
- G01N—INVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
- G01N33/00—Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
- G01N33/48—Biological material, e.g. blood, urine; Haemocytometers
- G01N33/50—Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
- G01N33/53—Immunoassay; Biospecific binding assay; Materials therefor
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K38/00—Medicinal preparations containing peptides
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61K—PREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
- A61K39/00—Medicinal preparations containing antigens or antibodies
-
- Y—GENERAL TAGGING OF NEW TECHNOLOGICAL DEVELOPMENTS; GENERAL TAGGING OF CROSS-SECTIONAL TECHNOLOGIES SPANNING OVER SEVERAL SECTIONS OF THE IPC; TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10—TECHNICAL SUBJECTS COVERED BY FORMER USPC
- Y10S—TECHNICAL SUBJECTS COVERED BY FORMER USPC CROSS-REFERENCE ART COLLECTIONS [XRACs] AND DIGESTS
- Y10S530/00—Chemistry: natural resins or derivatives; peptides or proteins; lignins or reaction products thereof
- Y10S530/82—Proteins from microorganisms
- Y10S530/825—Bacteria
Abstract
This invention relates to a new protein, designated Rib, and subfragments, multiples or variants thereof, which confers protective immunity against infection with many group B streptococcal strains, in particular those of serotype III. The invention includes a procedure for purification of the protein, a procedure for preparation of highly specific antibodies, a reagent kit, a DNA sequence encoding the protein and a pharmaceutical composition comprising the protein or fragments or variants thereof.
Description
WO 94/21685 PCT/SE94/00246 1 Protein Rib, a cell surface protein that confers immunity to many strains of the group B Streptococcus: process for purification of the protein, reagent kit and pharmaceutical composition This invention relates to a novel protein designated Rib (and subfragments, variants and multiples thereof) which confers immunity to most invasive strains of the group B Streptococcus, a procedure for purification of the protein, antibodies specific to the protein, a reagent kit and a pharmaceutical composition comprising the protein or fragments thereof.
During the last three decades, the group B Streptococcus has emerged as a major cause of neonatal disease in the Western world. In the United States alone, there are about 10,000 cases per year of invasive disease caused by this bacterium. These infections have an overall mortality of about 20%, and many of the infants that survive have permanent neurological sequelae. In view of these findings, a large effort has been made to find methods of prevention and treatment and to analyze the mechanisms by which group B streptococci cause infections.
About 20 of all women are vaginal carriers of the group B Streptococcus, and vertical transmission from the maternal genital tract is probably the most common source of infection in neonatal disease caused by this bacterium. However, only 1 to 2 of the infants that are colonized by the group B Streptococcus at birth are afflicted by serious infection. Other factors than exposure to the bacterium during birth must therefore contribute to the development of neonatal disease. Mothers of infected infants have significantly lower levels of antibodies to the type III capsule, which implies that these antibodies are important for protection against neonatal disease Baker,C.J. and D.L. Kasper, N. Engl. J. Med. 1976, 294:753 Group B streptococcal strains are divided into four major serotypes (la, Ib, II, and III) based on the structure of the polysaccharide capsule (Baker, J InfDis 1990. 161: 917).
Serotypes I, II, and III occur in roughly equal proportions among strains in the normal flora, but type III accounts for about two-thirds of all isolates from invasive infections. Since the capsule is a known virulence factor, it has been studied in considerable detail, in particular in type III strains. Efforts have been made to develop a vaccine, in which the type III polysaccharide capsule would be an essential component. However, use of the polysaccharide WO 94/21685 PCT/SE94/00246 2 capsule as a vaccine may give problems due to crossreactions with human tissues (Pritchard et al., Infect Immun 1992. 60: 1598). It would therefore be very valuable if one could develop a vaccine based on proteins rather than on polysaccharides.
The group B Streptococcus can also cause mastitis in cows, a bovine disease that is of considerable economical importance. Development of a vaccine against group B streptococcal infections is therefore of interest also in veterinary medicine.
STwo group B streptococcal cell surface proteins have previously been studied in detail: S the alpha and beta proteins. These proteins confer protective immunity to strains expressing the proteins, but they are of limited interest for group B streptococcal disease, since they are usually not expressed by type III strains, which cause the majority of serious infections.
.9 *9 9 9 Our invention relates to a streptococcal cell surface protein, and variants and subfragments thereof. This protein, which is designated protein Rib, was isolated from a group B streptococcal strain of serotype III as a distinct 95 kD protein. Protein Rib is expressed by almost all group B streptococcal strains of serotype III and by a few strains of other serotypes such as II. A method has been devised to purify protein Rib and it has been demonstrated that antibodies to this protein protect against lethal infection with strains expressing protein Rib.
The invention also relates to naturally occurring and artificially modified variants, subfragments and multiples thereof with ability to protect against infections caused by protein Rib expressing bacteria, i.e. especially group B streptococcal strains of serotype III.
:0 The invention also relates to a vector, such as a plasmid, a cosmid or a phage, .9 containing the genetic code for protein Rib and variants, subfragments and fragments thereof, suitable for insertion in a non-human host organism and expression from said host. The invention particularly relates to three phage clones, lambda Ribl-3, lambda Ribl-5 and lambda Ribl-7, having deposit numbers DSM. 9039, 9040 and 9041 respectively.
The invention also relates to a DNA sequence encoding protein Rib and variants, subfragments fragments and multiples thereof, that may be inserted in a suitable vector, such as a plasmid, a cosmid or a phage. The DNA sequence can be obtained from the deposited phages lambda Ribl-3, lambda Ribl-5 och lambda Ribl-7.
WO 94/21685 PCT/SE94/00246 3 The Rib protein is expressed by different type III strains. Extracts prepared from several different strains that were analyzed by Western blotting, using anti-Rib serum for the analysis, showed that almost all extracts contained protein Rib, but the molecular mass of the protein varied between 65 and 125 kD (data not shown). This result was not unexpected, since size variation has previously been described also for other group B streptococcal proteins, the alpha and beta proteins.
The available data suggest that the protein may consist of multiples of units, each unit corresponding to a molecular mass of about 9 kD. The invention therefore includes subfragments and multiples of the 95 kD protein or of a basic unit with the same characteristics. Variants include substitution or insertions of amino acids without changing the ability to protect against infections caused by bacterias expressing the protein.
Group B streptococcal strains are well known and may be isolated from the blood of infected human beings. The BM110 strain used by the inventors was obtained from Dr. S.
Mattingly University of Texas, San Antonio, Texas). All strains referred to herein are obtainable from the inventors at the University of Lund and the Lund University Hospital Doctor Gunnar Lindahl, Department of Medical Microbiology, S6lvegatan 23, S 22362 Lund, Sweden).
Protein Rib may be isolated from group B streptococcal strains of serotype III, preferably from strain BS30 or BM110. The invention concerns a process for purification of protein Rib.
The protein may be isolated by the following procedure: A Streptococcus Group B strain expressing the protein is cultivated, the medium and/or the microorganism are isolated, the bacteria are digested with an enzyme, preferably mutanolysin, a protease inhibitor is optionaly added, the digested bacteria are separated from the supernatant and protein Rib is extracted from the supernatant. The media can be any media suitable for cultivation of streptococci, such as Todd-Hewitt broth (Oxoid) and the cells are preferably cultivated 1-30, especially 12-20 hours. The digestion with an enzyme, preferably mutanolysin, is performed without shaking for 1-30, especially 10-20, preferably 15-18 hours at 20-40 preferably 37 The protein may be isolated from the medium, and in such a case there is no need for digestion with the enzyme which is used to break the cell walls. A protease inhibitor such as i,- WO 94/21685 PCT/SE94/00246 4 benzamidine chloride, iodoacetic acid or phenylmethyl sulfonyl fluoride is added to prevent the action from proteases which may contaminate the mutanolysin or may be present in the microorganisms.
The protein can be purified by ion exchange chromatography, preferably anion exchange chromatography and gel filtration, and fractions containing the protein collected according to established practice within the art.
The invention especially concerns a substantially pure protein Rib or subfragments thereof. With the expression "substantially pure" we understand a substance that does not contain pharmaceutically harmful substances.
The invention also concerns antibodies corresponding to protein Rib and subfragments, variants or multiples thereof. It is well known how to immunize an animal with an antigen, in this case protein Rib, collect the blood, isolate the serum and use the antibodies that react with the protein. The serum or an IgG fraction containing the antibodies may be used in analyzing the protein.
Since antibodies to protein Rib can protect against lethal infection with group B streptococcal strains, a method to measure the level of such antibodies can be valuable, for example in order to estimate if a pregnant woman has antibodies enough to protect the baby from such an infection. Protein Rib or subfragments thereof can be used to detect such antibodies to the protein. The invention therefore also concerns a reagent kit containing protein Rib or subfragments thereof.
It can also be of interest to analyze various samples for the presence of protein Rib.
Antibodies to the protein can be used for this purpose. The invention therefore also concerns a reagent kit, comprising antibodies to protein Rib or subfragments thereof, for detection of the protein. A reagent kit may contain any of the above mentioned blood fractions containing the antibodies. It may also contain the protein, subfragments or multiples thereof for use as a standard.
The properties of protein Rib indicate that this protein can be used for the development of a vaccine against the group B Streptococcus. The invention therefore also concerns a WO 94/21685 PCT/SE94/00246 pharmaceutical composition comprising the protein or fragments thereof as active ingredients, possibly together with pharmaceutically acceptable adjuvants and excipients. Suitable pharmaceutically acceptable adjuvants are those conventionally used in this field. Examples of suitable excipients are mannitol, lactose, starch, cellulose, glucose, etc., only to mention a few.
The examples given of the adjuvant and the excipients are not to be regarded as limiting the invention.
The invention will now be described in more detail, with the accompanying drawings, in which: Figure I shows a Western blot analysis of extracts prepared from group B streptococcal strains representing the four main serotypes (type la: strain A909; type Ib: SB35; type II: B1284; type III: BS30). As shown in the immunoblot, the strains of types la and Ib express the alpha and beta proteins, and the positions of these proteins in the stained gel are indicated by arrows (lower arrow: alpha antigen; upper arrow: beta antigen). The position in the stained gel of the protein Rib of the type III strain BS30 is indicated by a star. Molecular mass markers, indicated on the left, are in kD.
Figures 2A and 2B show purification of protein Rib from the type III strain BS30. A mutanolysin extract, partially purified through a previous step of DEAE ion exchange chromatography, was subjected to ion exchange chromatography on a 30 ml column of DEAE Bio-Gel A, which was eluted with a linear gradient (800 ml) of NaCI in 10 mM Tris, pH followed by 1 M NaCI (60 ml). The shaded area indicates fractions containing protein Rib. The insert shows a pool of the protein Rib-containing fractions analyzed by SDS-PAGE; molecular mass markers, indicated on the left, are in kD, and the position of protein Rib (95 kD) is indicated by an arrow. The pool of protein Rib-containing fractions from the ion exchange chromatography was subjected to gel filtration on a column (4.2 x 90 cm) of Sepharose CL6B.
The shaded area indicates fractions containing protein Rib and the insert shows a pool of these fractions analyzed by SDS-PAGE. Vo, void volume; Vt, total volume.
Figures 3A. 3B and 3C show analysis of group B streptococcal strains of the four major serotypes for cell surface expression of the alpha, beta and Rib proteins. Five strains were tested: A909 (type Ia); SB35 (type Tb); B1284 (type II); BS30 (type III), and BM110 (type III).
The symbols used for these five strains are shown in panel C. Bacterial suspensions were SUBSTITUTE SHEET I I I I WO 94/21685 PCT/SE94/00246 6 incubated with different dilutions of rabbit antiserum to the alpha, beta or Rib protein, as indicated. The numbers on the x-axis refer to final antibody dilution in the bacterial mixture.
Bound antibodies were detected by incubation with radiolabelled protein G. Controls with preimmune rabbit serum were included in all experiments and were completely negative in all cases.
Figure 4 shows Western blot analysis of purified alpha, beta, and Rib proteins with rabbit antisera raised against the purified proteins. Antisera were used at a 1:1,000 dilution, and bound antibodies were detected with radiolabelled protein G. Molecular mass markers, indicated on the left, are in kD.
Figure 5 shows SDS-PAGE analysis of the purified alpha, beta, and Rib proteins treated with trypsin or pepsin. The trypsin treatment was performed at pH 7.5, the pepsin treatment at pH The samples were neutralized before the SDS-PAGE analysis. Controls were treated in the same way as the samples containing trypsin or pepsin, but no enzyme was added; such treatment did not cause degradation of the proteins. P pepsin; T trypsin. Molecular mass markers, indicated on the left, are in kD.
Figures 6A. 6B and 6C show the results of cloning of the rib-gene from strain BM110 and expression of protein Rib in Escherichia coli. Western blot analysis of 7 different X clones.
Incubation with anti-Rib. Restriction digests of chromosomal DNA from strain BM110. (C) Restriction digests of the Rib expressing X-clone Xrib3.
Mutanolysin extracts of several strains of different serotypes were analyzed by SDS- PAGE and by immunoblotting, using antisera to the alpha and beta proteins, see example 1.
Results obtained with four strains representing the four major serotypes are shown in Fig. 1.
The alpha and beta proteins, which are expressed by both the type la strain and the type Ib strain, gave rise to distinct bands in the high molecular weight region of the stained gel. These proteins vary in size between the two strains, in agreement with previous observations. A major protein species in the high molecular weight region was present also in the extract prepared from the type III strain, although this strain does not express the alpha protein or the beta protein. Such a distinct protein species of high molecular weight was also observed in extracts of other type III strains, and the protein appeared to vary in size between different strains. These similarities to the alpha and beta proteins made it of interest to study the high SUBSTITUTE SHEET WO 94/21685 PCT/SE94/00246 7 molecular weight proteins of type III strains in more detail. Strain BS30 was chosen for this work, because it was known to be mouse virulent. The 95-kD protein expressed by this strain (Fig. 1) was purified (Example 2) from mutanolysin extracts, using two consecutive steps of ion exchange chromatography, followed by gel filtration (Fig. Fractions were analyzed by SDS-PAGE for presence of the 95-kD protein. When appropriate fractions from the gel filtration were pooled and analyzed, only two protein species were found: a major protein and a minor 90-kD protein (see insert in Fig. 2B). The 90-kD protein most likely represents a degradation product of the 95-kD protein, since these two proteins were later shown to have the same NH 2 -terminal sequence. The purified protein is referred to as protein Rib (resistance to proteases, immunity, group Antiserum to the 95-kD form of protein Rib was prepared by immunizing rabbits with slices cut out from SDS-PAGE gels.
To analyze whether protein Rib is a cell surface protein, strains representing the four major serotypes were tested for ability to bind anti-Rib serum (Fig. The five strains studied included the four strains described above and an additional type III strain, BMl10, which is a member of the high-virulence type III clone. For comparison, these five strains were also tested for expression of the alpha and beta proteins, using antisera to highly purified preparations of these proteins.
The anti-alpha serum reacted strongly with the la and Ib strains, as expected, and it also reacted weakly with the two strains of type III (Fig. 3A). However, mutanolysin extracts of the type III strains did not contain any detectable alpha protein, when analyzed in a Western blot.
It therefore seems likely that this weak reactivity of anti-alpha serum with whole bacteria of type III represents a cross-reactivity with some other cell wall component. These data show that reactivity with anti-alpha serum can be used to unequivocally analyze whether a strain expresses the alpha antigen on the cell surface. Similar data were obtained with anti-beta serum (Fig. 3B).
The antiserum to protein Rib reacted with the two type III strains, but not with the type Ia and Ib strains (Fig. 3C). An intermediate level of binding was observed for the type II strain. When mutanolysin extracts of the five strains were analyzed in a Western blot experiment, using anti-Rib serum for the analysis, the extracts of the type III strains reacted strongly, giving major blotting bands at 95 kD, but the extracts of the three other strains completely lacked reactivity (data not shown). This result indicates that the intermediate WO 94/21685 PCT/SE94/00246 8 reactivity of anti-Rib serum with the type II strain was due to a crossreactivity, which disappeared under the conditions of the Western blot. We conclude that protein Rib is expressed on the cell surface of the two type III strains, but not on the other three strains.
A total of 58 strains of known serotype, all of which had been isolated from invasive infections, were then tested for ability to bind antibodies to protein Rib (see Table 1, example Each strain was also tested for binding of antibodies to the alpha and beta proteins. To simplify the study of many strains, each antiserum was tested at a single 1000-fold dilution, chosen on the basis of the data shown in Fig. 3. This type of analysis gave unequivocal results, summarized in Table 1 of example 6. Protein Rib was found on the cell surface of 31 out of 33 type III strains and on one out of 13 type II strains, but not on any of the 12 strains of types la and Ib.
It seemed possible that strains lacking protein Rib on the cell surface excrete the protein into the medium. Culture supernatants of the 58 strains listed in Table 1 were therefore analyzed in a dot-blot experiment, using anti-Rib serum for the analysis. Protein Rib was not detected in the supernatants of any of the 26 strains that do not express the protein on the cell surface, but was found in the supernatants of 26 of the 32 strains expressing the protein on the cell surface (data not shown).
A mouse protection model was used to study whether rabbit antibodies to protein Rib can protect against lethal infection with the group B Streptococcus (Table 2, Example 7).
Control animals received antiserum to the alpha protein or preimmune serum, as indicated. The data show that antiserum to protein Rib protects mice against lethal infection with strains expressing protein Rib.
Since protein Rib confers protective immunity, like the alpha and beta proteins, it was of interest to compare these three proteins. A Western blot experiment was performed, using antisera to the purified proteins for the analysis (Fig. The staining gel showed that the three proteins were highly purified, with one major species in each preparation, but there was no serological cross-reaction between the three proteins, as shown in the Western blot.
The alpha and beta proteins were originally distinguished due to a difference in protease sensitivity. The alpha protein is resistant to trypsin but sensitive to pepsin, while the beta b WO 94/21685 PCT/SE94/00246 9 protein is sensitive to both of these proteases (Bevanger and Maeland, Acta Path Microbiol Scand Sect B 1979. 87:51). An experiment with the purified alpha and beta proteins confirmed this difference and also demonstrated that protein Rib is resistant to both trypsin and pepsin (Fig. As expecterc all three proteins were sensitive to degradation by proteinase K (data not shown). The protease 'esistance of protein Rib was not due to the presence of an inhibitor, since beta protein was completely degraded by both trypsin and pepsin even in the presence of protein Rib (data not shown).
The invention will now be described with the following examples, which however do not limit the scope of the invention.
EXAMPLE 1. IDENTIFICATION OF THE PROTEIN Four group B streptococcal strains representing the four main serotypes were used as reference strains: A909, type la/c; SB35, type Ib; B1284, type II; BS30, type III, described here. The BS30 strain was isolated at Lund University Hospital from a boy with neonatal infection. All bacterial strains were grown in Todd-Hewitt broth (Oxoid) at 37 0 C, without shaking. Mutanolysin extracts of the strains were analyzed by SDS-PAGE and by immunoblotting using antisera to the alpha and beta proteins. Small-scale mutanolysin extracts of streptococcal strains were prepared as described for the large-scale extracts used for protein purification, but cultures of only 50 ml were used to prepare 20% bacterial suspensions, of which 1 ml samples were digested with the enzyme.
SDS-PAGE was performed with standard techniques, using a total polyacrylamide concentration of 10% and a cross-linking of Samples were boiled for 3 min in a solution containing 2% SDS and 5% 2-mercaptoethanol prior to electrophoresis. The separated proteins were stained with Coomassie Brilliant Blue R-250 or transferred by electroblotting to a membrane of methanol-activated polyvinylidene difluoride (Immobilon-P; Millipore Corp., Molsheim, France), using a Semi-Dry Electroblotter (Ancos, Vig, Denmark). The Immobilon membranes were blocked with gelatin, using standard procedures, and then incubated with the indicated type of rabbit antiserum diluted 1000-fold see example 7 followed by radiolabelled protein G and autoradiography.
I I WO 94/21685 PCT/SE94/00246 Proteins were radiolabelled with carrier-free 2 I (Amersham International, England), using the chloramine T method. Total protein concentrations were determined with the MicroBCA protein assay reagent (Pierce). Electroelution of protein from SDS-PAGE gels was performed with a model 422 Electro-Eluter from Bio-Rad.
The results are shown in fig. 1.
EXAMPLE 2. PURIFICATION OF PROTEIN Rib The bacteria in a 10 1 overnight culture of strain BS30 were spun down, washed twice with 50 mM Tris, pH 7.3, and resuspended to 20% in the same buffer. Mutanolysin (Sigma Chemical Co., St. Louis, MO), dissolved to 5000 units/ml in 10mM potassium phosphate, pH 6.2, was then added to the bacterial suspension (125 ml) to give a final concentrati -n of 350 units/ml. The digestion was allowed to proceed for 17 h at 37 0 C with gentle shaking, and protease inhibitors were then added to the following final concentrations: benzamidine chloride, 5 mM; iodoacetic acid, 5 mM; phenylmethyl sulfonyl fluoride, 2 mM.
The suspension was centrifuged and the supernatant was immediately dialyzed dialysis tubing Spectrapor No. 4) against 10 mM Tils, pH 8.0. This dialyzed preparation was subjected to two consecutive steps of ion exchange chromatography, which allowed the best recovery of pure protein Rib, as shown by preliminary experiments. The presence of protein Rib was analyzed by SDS-PAGE and visual inspection of the gels for the presence of the 95-kD band. In the first chromatography step, the dialyzed preparation (110 ml) was mixed with the same volume of 0.4 M NaCI in 10 mM Tris, pH 8.0 and 30 ml of DEAE Bio-Gel A (BioRad Laboratories, Richmond, CA), equilibrated with 10 mM Tris, pH 8.0. This mixture was stirred gently at 4°C for 1 h, and unabsorbed material (containing protein Rib) was freed from the gel by filtration through a glass filter. For the second chromatography step (Fig. 2A), the filtrate containing protein Rib was diluted twenty-fold with distilled water, to reduce the ionic strength, and mixed with 30 ml of DEAE Bio-Gel A, equilibrated as described above. After gentle stirring at 4°C for 16 h, the gel was recovered by filtration and washed with 10 mM Tris, pH Absorbed proteins (including protein Rib) were eluted with an 800 ml linear salt gradient (0 0.2 M NaCI in 10 mM Tris, pH followed by 1 M NaCI (60 ml). Fractions (10 ml) were collected and those containing protein Rib were pooled, concentrated, and subjected to gel -s~C II WO 94/21685 PCT/SE94/00246 11 filtration in a column of Sepharose CL6B (4.2 cm x 90 cm) iri PBSA (0.12 M NaCI, 0.03 M phosphate, 0.02 NaN 3 pH 7.2) (Fig. 2B). The fractions were analyzed by SDS-PAGE electrophoresis for presence of the 95-kD band. Fractions (10 ml) containing protein Rib were pooled and frozen. The yield of protein Rib was about 6 mg from 25 g of bacteria. To ensure the purity of the protein Rib preparations used for immunochemical analysis, the protein used for such work was further purified by SDS-PAGE, followed by electroelution of the band. However, SDS-PAGE analysis did not demonstrate any difference in purity between this electro-eluted material and that recovered from the gel filtration step.
As mentioned above, protein Rib is also found in the medium of strains expressing the protein. The protein can be purified from such a medium, using techniques similar to those described above.
Automated amino acid sequence analysis of protein bands transferred to Immobilon was performed directly on the membranes, using an Applied Biosystems 470A gas-liquid solidphase sequenator. The membranes were lightly stained with Coomassie Brilliant Blue to localize the protein bands, which were then cut out for sequencing. The SwissProt Data Bank was used for analysis of protein sequences.
The NH 2 -terminal sequence of protein Rib from strain BS30 is shown in SEQ ID NO:1.
The two proteins with estimated molecular masses of 95 kD and 90 kD ;in s'-rified protein Rib (Fig. 2B) were found to have the same NH_-terminal sequence, suggestiri Iat the smaller molecule is a degradation product of the larger one. A data search showed that the NH,terminal sequence of protein Rib is unique.
The same purification procedure was also followed for the isolation of protein Rib from strain BM110. The NH 2 -terminal sequence (SEQ ID NO:2) of protein Rib isolated from strain BM 110 may differ from the NH2-terminal sequence of the corresponding protein from BS30 at position 7, where the BM110 protein may have Ser in place of Asp.
EXAMPLE 3. PURIFICATION OF THE ALPHA PROTEIN The alpha protein was purified from strain SB35, a type Ib strain expressing both the alpha and beta proteins. The procedure used was similar to that used for purification of protein WO 94/21685 PCT/SE94/00246 12 Rib from strain BS30. Fractions were analyzed for the presence of alpha protein by dot-blot analysis, using rabbit anti-alpha serum (kindly provided by Dr. L. Bevanger, University of Trondheim, Norway) and protein G (Calbiochem Co., San Diego, CA) radiolabelled with 1'I.
In the ion exchange and gel filtration steps, the behaviour of the alpha protein was similar to that of protein Rib (cf. Fig. The alpha protein recovered from the gel filtration step was present in a sharp peak. Analysis of this material with different antisera indicated that it contained trace amounts of contaminating beta protein, which was removed by passage of the preparation through a small column of IgA-Sepharose. The purified alpha protein had a molecular weight of about 110,000, according to SDS-PAGE analysis (cf. Fig. The yield of alpha protein was 12 mg from 39 g of bacteria. The alpha protein used for immunochemical work was further purified by electroelution from SDS-PAGE gels, as described above for protein Rib. However, SDS-PAGE analysis did not demonstrate any difference in purity between this electro-eluted material and that recovered from the gel filtration step.
EXAMPLE 4. PURIFICATION OF THE BETA PROTEIN The IgA-bitiding beta protein (Russell-Jones et al, J Exp Med 1984. 160: 1467) was purified by a procedure similar to that used for the Rib and alpha proteins. The starting material was obtained by incubating washed SB35 bacteria in 50 mM glycine-NaOH buffer, pH 11.0 (final pH in suspension Previous work in our laboratory had shown that the major protein species in such an extract is the beta protein. The extract (222 ml) was immediately dialyzed against 10 mM Tris, pH 8.0, diluted twenty-fold with distilled water and mixed with ml of DEAE Bio-Gel A (equilibrated with 10 mM Tris, pH After gentle stirring at 4°C for 2 h, the gel was transferred to a column and eluted with an 800 ml linear salt gradient (0 0.2 M NaCI in 10 mM Tris, pH A dot blot procedure was used to test fractions ml) for presence of beta protein, using radiolabelled IgA or anti-beta serum and radiolabelled protein G for the analysis. The beta protein was eluted in the first part of the gradient.
Appropriate fractions were pooled, concentrated, and subjected to gel filtration on a column (4.2 x 100 cm) of AcA34 (Pharmacia-LKB, Uppsala, Sweden) in PBSA. The beta protein was eluted in a well-defined peak. Appropriate fractions were pooled, concentrated and frozen. The yield was 9 mg of pure protein from 23 g of bacteria.The major protein species in such a preparation had a molecular weight of about 130,000, according to SDS-PAGE, but small amounts of degradation products of lower molecular weight were also seen when the protein was subjected to Western blot analysis.
1 -1 WO 94/21685 PCT/SE94/00246 13 EXAMPLE 5. ANALYSIS OF PROTEASE SENSITIVITY For analysis of protease sensitivity (Fig. 200 pl samples of purified alpha, beta or Rib protein (0.5 mg/ml) were incubated for 1 h at 37 0 C with trypsin, pepsin, or proteinase K (0.2 mg/ml). Trypsin digestion was performed in 0,25 M sodium phosphate, pH 7.5, pepsin digestion in 0.25 M sodium acetate, pH 4.0, and proteinase K digestion in 0.25 M Tris, pH 7.4. The samples were neutralized before analysis by SDS-PAGE.
EXAMPLE 6. ANALYSIS OF STREPTOCOCCAL STRAINS FOR CELL SURFACE EXPRESSION OF THE ALPHA. BETA AND Rib PROTEINS Five reference strains available in our laboratory were first analyzed for surface expression of the alpha, beta and Rib proteins. Later, a collection of 58 group B streptococcal strains, all isolated from cases of invasive infections, were also used to study the expression of these cell surface proteins (see Table Typing of group B streptococcal strains was performed in the Clinical Microbiology Laboratory of Lund University Hospital, using standard techniques.
The bacteria in a 10 ml overnight culture were washed twice with PBSAT (PBSA supplemented with 0.05% Tween 20) and a 1% suspension in PBSAT was prepared. A sample (180 l) of this bacterial suspension was mixed with 20 1l of rabbit antiserum that had been diluted in PBSAT and the mixture was incubated at 23 0 C for 1 h. Two ml of PBSAT were then added, the bacteria were spun down, washed once with 2 ml of PBSAT, and resuspended in 200 1l of PBSAT. For detection of bound IgG, 25 /l of radiolabelled protein G about cpm in PBSAT) was then added and incubation was continued at 23°C for 1 h. Following addition of 2 ml of PBSAT, the bacteria were spun down and the pellet was then washed by addition of 2 ml of PBSAT. After a final centrifugation, the supernatant was discharged and the radioactivity in the pellet was determined. When many strains were tested for expression of the alpha, beta and Rib proteins (Table a single final antiserum dilution of 1:1,000 was used Controls with preimmune rabbit antiserum were always included and were completely negative in all cases. Protein Rib was found on the cell surface of 31 out of 33 type III strains, but not on any of the 12 strains of types la and Ib.
I
WO 94/21685 PCT/SE94/00246 14 Table 1. Cell surface expression of the alpha, beta and Rib proteins by 58 group B streptococcal strains isolated from patients with invasive infections Capsular type Protein expressed Ia (n=9) Ib (n=3)
II
13)
III
(n=33) alpha beta alpha and beta Rib none The cell surface expression of the alpha, beta, and Rib proteins was analyzed with specific antisera, and bound antibodies were detected with radiolabelled protein G, as shown in Figure 3.
"The 58 strains studied here were all isolated from cases of invasive infections, but do not represent a random collection of such strains, since most of the type II strains were later added to the collection originally studied, which included only two type II strains.
WO 94/21685 PCT/SE94/00246 EXAMPLE 7. PREPARATION OF ANTISERA AND MOUSE PROTECTION TESTS All antisera were produced in rabbits, which were immunized s.c. on the back. For preparation of antiserum to protein Rib expressed by strain BS30, slices corresponding to several 95 kD bands in SDS-PAGE gels were cut out, divided into small pieces and mixed with complete Freund 's adjuvant. For the initial immunization, six slices (about 60 /g of protein) in 1 ml of PBS were mixed with 1 ml of adjuvant. Three bands (30 /g of protein) were used for booster injections. The first booster was given after 4 weeks and 3 additional boosters were given with intervals of 2 weeks. The rabbit was then bled 3 times with intervals of 3 weeks; the serum obtained from these 3 bleedings was pooled and used for the experiments reported here. Antiserum to the alpha protein was prepared by the same procedure. The first sample of anti-alpha serum, used to analyze fractions during the purification, was obtained from Dr Lars Bevanger, Trondheim. Antiserum to the purified beta protein was available in our laboratory.
C3H/HeN mice, bred in our department, were used at an age of 10-20 weeks. The mice were injected i.p.with 0.5 ml of a rabbit serum diluted five-fold in PBS, and infected 4 h later by i.p. injection of 0.5 ml of log-phase bacteria diluted in Todd-Hewitt broth. The number of bacteria used, which was estimated to be the 90% lethal dose (LDg), was 2 x 106 c.f.u. for strains BM110, BE210, and SB35sedl, and 2 x 107 c.f.u. for BS30 and L25. Dead animals were counted daily for 4 days. Control animals usually died within 24 h.
WO 94/21685 PCT/SE94/00246 16 Table 2. Rabbit antiserum to protein Rib protects mice against lethal infection with group B streptococcal strains expressing this protein Strain Capsular type Relevant cell surface protein" Mice survivingt after pretreatment with anti-Rib serum anti-alpha serum normal serum III Rib 29/32' 1/15 BM110 III Rib 15/24' 0/15 III 0/15 2/14 BE210 II Rib 10/151 0/14 I Ib alpha 1/15 10/15- 4/20 0/15 n.d.ll n.d.
n.d.
C3H/HeN mice were injected i.p. with 0.1 ml of rabbit antiserum (diluted to 0.5 ml with PBS) and challenged 4 h later with an LD dose of log-phase bacteria, diluted into 0.5 ml of Todd-Hewitt broth. The survival data were analysed by the chi-square test.
Expreuio of protein Rib or the alpha protin, the two antigens relevant to these experiments t No. of mice surviving for 4 days total no. of infected mice P 0.001 when compared to the controls receiving anti-alpha serum or normal serum n.d. not determinated 'P<0.001 when compared to the controls receiving anti-alpha serum "P<0.01 when compared to the controls receiving anti-Rib serum I ,II WO 94/21685 PCT/SE94/00246 17 The data in Table 2 demonstrate that antiserum to protein Rib protects against lethal infection with BS30, the type III strain from which the protein had been purified. This protection is not unspecific, as shown by the experiments with control sera. The anti-Rib serum also protected against lethal infection with another type III strain, BM110, a member of the high-virulence clone of group B streptococcal strains (Musser et al., Proc. Natl. Acad. Sci USA 1989. 86: 4731) In contrast, the anti-Rib serum did not protect against infection with one of the type III strains that do not express protein Rib (Table The protective effect of anti-Rib serum was not limited to type III strains, as shown by the experiments with a type II strain expressing protein Rib. As expected, anti-Rib serum did not protect against a type Ib strain expressing the alpha antigen. Taken together, these data strongly suggest that protein Rib acts as a virulence factor in almost all type III strains and in some type II strains, i.e. in most group B streptococcal strains causing invasive infections.
EXAMPLE 8. CLONING OF THE rib-GENE AND EXPRESSION OF PROTEIN RIB IN ESCHERICHIA COL.
The structural gene for protein Rib was cloned from strain BM110, a serotype III strain which is a member of a high-virulence clone. Protein Rib expressed by this strain (SEQ ID NO:2) and protein Rib expressed by strain BS30 (SEQ ID NO: 1) have similar size and NH 2 terminal sequence. A library of strain BM110 DNA in bacteriophage lambda was constructed.
The bacteria in a 500 ml log-phase Todd-Hewitt culture of the strain BM110 were spun down.
The pellet was frozen and thawed 3 times, suspended in 20 ml TE buffer (10 mM Tris, ImM EDTA pH centrifugated, washed and resuspended in 4 ml of the same buffer.
Mutanolysin (Sigma Chemical Co. St Louis, MO, USA) dissolved to 5000 units/ml in 10 mM potassium phosphate, pH 6.2, was added to the bacterial suspension to give a final concentration of 500 units/ml. Lysozyme (Sigma) was added to a final concentration of 8 mg/ml, and the digestion was allowed to proceed for 3 h at 37 oC. The bacterial cells were lysed by addition of 200 /l of 10 SDS and 500 Il Tween lysing mix (2 Tween-20, mM Tris pH 8.0 and 60 mM EDTA), followed by another 200 pl of 10 SDS. The lysate was treated with proteinase K (Sigma, 100 ug/ml) for 19 h at 50 oC, followed by repeated phenol and chloroform extractions. The DNA was precipitated with ethanol, dried in a SpeedVac concentrator (SAVAC) and dissolved in 4.5 ml TE buffer. The DNA was further I I 18 purified by CsCl density gradient ultracentrifugation and dialysed against TE buffer. The DNA concentration was then approximately 2.5 This DNA was partially digested with Sau 3AI (Promega), and ligated to Bam HI-cleaved arms of XEMBL 3 (Stratagene). The recombinant phage DNA was packaged in vitro using Gigapack II Gold Packaging Extract (Stratagene). The library was plated on the E. coli strain LE392 and screened for production of protein Rib with an immuno-blotting technique: plates with about 1000 plaques Swere covered with a nitrocellulose membrane and left at 4°C for 1 h. The membranes were removed, blocked, and incubated in buffer containing rabbit anti-Rib serum, diluted fold. Positive plaques, i.e. those binding rabbit IgG, were detected by addition of peroxidase-labeled protein A (Sigma) (20 p/ml) and the presence of peroxidase was visualized, using standard techniques. Seven independent Rib expressing lambda clones were isolated. Three of these clones, i.e. lambda Rib 1-3, lambda Rib 1-5 and lambda Rib were deposited at Deutsche Sammlung von Microorganismen Mascheroder Weg Ib D-38124 Braunschweig Germany on 16 March 1994 and accorded deposit numbers DSM 9039, 9040 and 9041 respectively. A preparation of DNA from the lambda Rib 1-3 clone having a DNA concentration of about 0.5 pg/pl was also made. Lysates of these seven clones were subjected to Western immunoblot analysis, using anti-Rib serum (see figure Several of the clones express protein Rib of the same size as protein Rib isolated directly from strain BM110.
Example 9 DNA Sequencing and Sequence Analysis DNA sequences were determined by the dideoxy chain termination method using [a- 35 S]dATP (Amersham Corp.) and Sequenase 2.0 (Amersham Corp.). Recombinant M13mp 18 or Ml3mpl9 phage DNA was used as template. M13 universal primer and -40 primer (Amersham Corp.) as well as custom made primers were used. The sequencing reaction products were resolved on 8% polyacrylamide-urea gels. Gels were \\HELBO\home\Sharon\KepkspeC1\638.4 doc 28/06I97 ill 18a run at 40 W for 1-4 h on a sequencing unit for Cambridge Electrophoresis Ltd. (Cambridge, UK), fixed in methanol, 10% acetic acid for 15 min, and dried on Whatman 3MM papers under vacuum. Computer-assisted analysis of DNA was performed with the GCG software package (16) and the Gene Works program (IntelliGenetics, Inc., Mountain View, CA). The Complete DNA sequence and deduced amino acid sequence are set out in SEQ ID NO:3 and SEQ ID NO:4 respectively.
\\MELBOI\homeS\Shiron\KeeP\sPec1\681 .94.doc 2810t9l WO 94/21685 SEQUENCE LISTING GENERAL INFORMATION:
APPLICANT:
NAME: Gunnar Lindahl STREET: Magnus Stenbocksgatan CITY: Lund COUNTRY: Sweden POSTAL CODE (ZIP): 222 24 (ii) TITLE OF INVENTION: Protein Rib, a cell surface protein that confers immunity to many strains of the group B Streptococcus: process for purification of the protein, reagent kit and pharmaceutical composition.
(iii) NUMBER OF SEQUENCES: 2 (iv) COMPUTER READABLE FORM: MEDIUM TYPE: Floppy disk COMPUTER: IBM PC compatible OPERATING SYSTEM: PC-DOS/MS-DOS SOFTWARE: Patentln Release Version #1.25 (EPO) CURRENT APPLICATION DATA: APPLICATION NUMBER: INFORMATION FOR SEQ ID NO:1: SEQUENCE CHARACTERISTICS: LENGTH: 12 amino acids TYPE: amino acid TOPOLOGY: linear (ii) MOLECULE TYPE: protein (iii) HYPOTHETICAL: NO (iv) ANTI-SENSE: NO FRAGMENT TYPE: N-terminal (vi) ORIGINAL SOURCE: ORGANISM: Streptococcus group B STRAIN: (xi) SEQUENCE DESCRIPTION: SEQ ID NO:1: Ala Glu Val lie Ser Gly Asp Ala Val Thr Leu Asn 1 5 INFORMATION FOR SEQ ID NO:2: SEQUENCE CHARACTERISTICS: LENGTH: 12 amino acids TYPE: amino acid TOPOLOGY: linear PCT/SE94/00246 (ii) MOLECULE TYPE: protein 20 (ij i) (v (vi) HYPOTHETICAL: NO FRAGMENT TYPE: N-terminal ORIGINAL SOURCE: ORGANISM: Streptococcus group B STRAIN: BM110 SEQUENCE DESCRIPTION:SEQ ID NO:2 Ala Glu Val Ile Ser Gly Ser Ala Val Thr Leu Asn 1 5 (xil) INFORMATION FOR SEQ ID NO:3 SEQUENCE CHARACTERISTICS: LENGTH: 3825 nucleotide TYPE: nucleotide TOPOLOGY: linear (ii) MOLECULE TYPE: protein (iii) HYPOTHETICAL: NO FRAGMENT TYPE: N-terminal (vi) ORIGINAL SOURCE: ORGANISM: Streptococcus group B STRAIN: BM110 (xi) SEQUENCE DESCRIPTION: SEQ ID NO:3 1 AATATTTGTT TTTAAAGCCT ATACTTTACT ATGTATAGAG
CTATACAGAA
51 TAAAGTAAAG GAGAATATTA TGTTTAGAAG GTCTAAAAAT
AACAGTTATG
101 ATACTTTACA GACGAAACAA CGGTTTTCAA TTAAGAAGTT
TAAGTTTGGT
151 GCAGCTTCTG TACTAATTGG TATTAGTTTT TTAGGAGGTT
TTACTCAAGG
201 GCAATTTAAT ATTTCTACAG ATACTGTGTT TGCAGCTGAA
GTAATTTCAG
251 GAAGTGCTGT TACGTTAAAC ACAAATATGA CTAAAAATGT
TCAGAATGGT
301 AGAGCATATA TAGATTTATA TGATGTGAAA AATGGGAAAA
TAGATCCATT
\\MELBOI\homeS\Sharol\Kefp\Spe :ci63S91.
9 4 .doc 28/05/97 21 351 ACAATTAATT T1A TG TCAT TA 401 GGCAAGGCGG
T)'ACTC;TTGGT
451 GOAGOTAGTA G-TC CT CATAC 501 GAAGCCTGAT
ACTATTTACA
551 ATTOTTCAGC GAAAG CGGAA 601 GACCCTAAAT
TAAGTTTAGA
651 TGATATCAAA 2 0 TCAGACATTG 701 CCAATAAAAT
AGTACCTCGA
751 ATCCCAGATG AGC AAGT CAA 801 TGTAGGTGAG
TTACCAGATC
851 TTCCGAAAGG
TACGGCAACA
901 CCGGGAGACA
ATGGTTCAAA
951 AGATACTGTA
ACAGATGCCG
1001 ATAAGAATGA
AGGTGAGACA
1051 CCGAAGGCAG
CGAAAGGTAC
1101 AACAGTAGCC
GGAGACAAAC
1151 CAGCAAAAGT
TACTGTAGAT
ACGTTAAATT
CAATTATTTC
TTAATTATAC
GGACAAGTGG
TTT GAGAG0AT
GGGAOGAGGG
ACAGATATTG
AACTGAJ\GTT
CCGATAAGAA
ACACCGAAGG
TAO AlACAG TA
AACCAGCAAA
GATGTGACTG
TCCAGCAGGT
AAGATTCTAT
TTTGAAACTC
TGTTGTGACT
CACCTGATTT
ACACAACCTT
AGTATTG AAG
ATATTATAAA
AAAATAGATG
AAGTCGCGAT
ATAATAA TOO AC TAATTTAG
TGATOCACCA
CAGAAGATTO
GOCTTTGAAA
AGTTGTTGTG
TTA.AGGTTGT
AAAGATOAGO
TGGTAAOT TA
OAGTTGATAO
TAOOOAGATG
AAAAGCTOAG
CTGAATTGAO
AOAGATGGAA
OGTTTOATTG
AAGTTAAAAA
AAAGTTTTGA
TAA GAOGOAA
AAAAAATAOT
GGTAAAGATO
TATTGGTAAO
OTOOAGTTGA
AOT TAO OCAG
OGATOOAOGT
AAGTOAATGT
OCAGATOTTO
GGOAAOAOOG
GTT OAAAAGA \\tELBOI\homeS\Sharn\KeeP\spec1\63891 .94.doc 28/05t97 22 1201 GTGACTGTTA AGGTTGTCGA TCCGCGTACA GATGCCGATA
AGAATGATCC
1251 AGCAGGTAAA
AAGGCAGAAG
1301 ATTCTATTGG AGT AG CCTTT 1351 GAAACTCCAG :AAAAGT TG T 1401 TIGTGACTrTAC 1451 TTGTCGATCC
AGGTAAAGAT
1501 CAGCAAGTCA
('TATTGGTAA
1551 CTTACCAGAT AC TCCAG T TG 1601 ATACGGCAAC C A(77T TAC CCA 1651 GATGGTTCAA T CGATCC GC G 1701 TACAGATGCC C AAG TCAATG 1751 TAGGTGAGAC
ACCAGATCTT
1801 CCGAAAGGTA
CGGCAACACC
1851 GGGAGACAAA G GT TCAAAAG 1901 ATACTGTAGA
AGATGCCGAT
4 1951 AAGAATGATC
GTGAGACACC
2001 GAAGGCAGAA
AAAGGTACAA
GATCAGCAAG
TAACTTACCA
TTGATACGGC
CCAGATGGTT
GCGTACAGAT
ATGTAGGTGA
C TTCCGAAAG
ACCGGGAGAC
AAGATACTGT
GATAAGAATG
ACCGAAGGCA
CAACAGTAGC
C CAGCAAAAG
TGTGACTGTT
CAGCAGGTAA
GATTCTATTG
TCAATGTAGG
GATCTTCCGA
AACAC CGGGA
CAAAAGATAC
GCCGATAAGA
GACACCGAAG
GTACAACAGT
AAACCAGCAA
AGATGTGACT
ATCCAGCAGG
GAAGATTCTA
CTTTGAAACT
TTGTTGTGAC
AAGGTTGTCG
AGATCAGCAA
GTAACTTACC
TGAGACACCG
AAGGTACAAC
GACAAACCAG
TGTAGATGTG
ATGATCCAGC
GCAGAAGATT
AGCCTTTGAA
AAGTTGT TGT
GTTAAGGTTG
TAAJXGATCAG
TTGGTAACTT
CCAGTTGATA
TTACCCAGAT
ATCCGCGTAC
GT CAATGTAG
AGATCTTCCG
0 I r: \\MEBOIhomS\ShronRee~speI\68q,94doc 2f0/05/97 2051) CAGTAGCGTT /\f/\,A/AACCA 1 GCAJ\AAGTTG L, I2fIAGjATGT 151 GACTGTTAAG '2AT C: GFAG 1( '201 CAGGTAAAGA
(;(GC(A(GAAGAT
51TCTATTGGTA
'TAGCCTTTGA
2301 AACTCCAGTT AAAG T TGTT G 2351 TGACTTACCC.
GTTAAGGTT
2401 GTCGATCCGC 2t"AAAGATCA 2451 GCAAGTGAAT
ATTGGTAACT
2501 TACCAGATCT 'FCC CAG TTGAT 2551 ACGGCAACAC CTT AC CCAGA 2601 TGGTTCAAAAA 2651 CAGATGCCGA
AGTCAATGTA
410 2701 GGTGAGACAC CAGAT OTTC0 2751 GAAAGGTACA
GCAACACCGG
2801 GAGAOAAACC T T CAAAAGAT 2 3
TGAAACTCCA
PU GTGACTTA
GTTGTCGATC
TCAGOAAGT 0
AOTTACCAGA
GATACGGCAA
AGATGGTTCA
GTACAGATGC
GTAGGTGAGA
TCCGAAAGGT
CGGGAGAOAA
GATAOTGTAG
TAAGAATGAT
CGAAGGCAGA
ACAGTAGCCT
AGCAAAAGTT
GTTGATACGG
CC CAGAT GGT
CGCGTACAGA
AATGTAGGTG
TO TTCCGAAA
CACCGGGAGA
AAAGATACTG
CGATAAGAAT
CACCGAAGGC
ACAACAGTAG
ACCAGCAAAA
ATGTGACTGT
CCAGCAGGTA
AGATTCTATT
TTGAAACTCC
GTTGTGACTT
CAACACCGGG
TCAAAAGATA
TGCCGATA AG
AGACACCGAA
GGTACMACAG
CAAACCAGCA
TAGATGTGAC
GATCCAGOAG
AGAAGATTCT
CCTTTGAAAC
GTTGTTGTGA
TAAGGTTGTC
AAGATCAGCA
GGTAACTTAC
AGTTGATACG
ACCCAGAT GG C3 2851 ACTGTAGATG TGACTGTTAA GGTTGTCGAT CCGCGTACAG AT GOCCGATAA \\MELBI&\homS\Sh.aronMkeep\speci\6' ,.94.doc 28105/97 24 2901 GAATGATCCA GCAGGTAAAG ATCAGCAAGT CAATGTAGGT
GAGACACCGA
2951 AGGCAGAAGA
AGGTACAACA
3001 GTAGCCTTTG
ACAAACCAGC
3051 AAAAGTTGTT
GTAGATGTGA
3101 CTGTTAAGGT
TGATCCAGCA
3151 GGTAAAGATC
CAGAAGATTC
3201 TATTGGTAAC
GCCTTTGAAA
3251 CTCOAGTTGA
AGTTGTTGTG
3301 ACTTACCCAG
TTAAGGTTGT
3351 CGATCCGCGT
AAAGATCAGC
3401 AAGTCAATGT
TGGTAACTTA
3451 CCAGATCTTC
CAGTTGATAC
3501 GGCAACACCG
TACCCAGATG
3551 GTTCAAAAGA
TCCGCGTACA
3601 GATGCCGATA
'PCAATGGTAA
3651 AGGAAATAAA
TTCTTTAATG
3701 TTGTAGCTTT
TGTTTCTAAG
TTCTATTGGT
AAACTCCAGT
GTGACTTACC
TGTCGATCCG
AGCAAGTCAA
TTACCAGATC
TACGGCAACA
ATGG TTCAAA
ACAGATGCCG
AGGTGAGACA
CGAAAGGTAC
GGAGACAAAC
TACTGTAGAT
AGAATGATCC
CTACCAGCAA
GACAATTATG
AACT TACCAG
TGATACGGCA
CAGATGGTTC
CGTACAGATG
TGTAGGTGAG
TTCCGAAAGG
CCGGGAGACA
AGATACTGTA
ATAAGAATGA
CCGAAGGCAG
AACAGTAGCC
CAGCAAAAGT
GTGACTGTTA
AGCAGGTAAA
CAGGTGAGAA
TCATCAGTTG
ATCTTCCGAA
ACACCGGGAG
AAAAGATACT
CCGATAAGAA
ACACCGAAGG
TACAACAGTA
AACCAGCAMA
GATGTGACTG
TCCAGCAGGT
AAGATTCTAT
TTTGAA.ACTC
TGTTGTGACT
AGGTTGTCGA
GATCAGCAAG
TGCAACTCCA
GTTTATTATC
\\MELBOheS\Sharon\eep\speCtt\ 6 38 9 1 .94.doc 28/05/91 3751 AAAAAAGAGG ATTAATCTTT TGACCTAAAA TGTCACTAAA
CTTTTCACCA
3801 TTTATTGGTG TGAACACATT AATAA INFORMATION FOR SEQ ID NO:4 SEQUENCE CHARACTERISTICS: LENGTH: 1231 amino acids TYPE: amino acid TOPOLOGY: linear (1i) MOLECULE TYPE: protein (iii) HYPOTHETICAL: NO FRAGMENT TYPE: N-terminal (vi) ORIGINAL SOURCE: ORGANISM: Streptococcus group B STRAIN: BM110 (xi) SEQUENCE DESCRIPTION: SEQ ID NO:4 1 MFRRSKNNSY DTLQTKQRFS
FTQGQFNIST
51 DTVFAAEVIS I DPLQLITLN 101 SPDLKAQYVI S PHTK PDGQ V
DIINVSLTIY
ISLDDIKTDI
201 DNNPKTQSDI
QQVNVGETPK
251 AEDSIGNLPD
DGSKDTVDVT
301 VKVVDPRTDA
PKGTTVAFET
351 PVOTATPGDK KN DPAGKDQQ 401 VNVGETPKAE AKVVVTY PDG 451 SKDTVDVTVK -1,SIGNLPDLPK
GSAVTLNTNM
RQGGNYFTQP
NSSALRDKI D
ANKITEVTNL
L PKGTT VA FE
DKNDPAGKDQ
PAKVVVTY PD
DSIGNLPDLTP
VVDPRTDADK
IKKFKFGAAS
TKNVQNGRAY
S ELTTVGAAS EVKKKAE DPK
EKILVPRIPD
TPVDTATPGD
QVNVGETPKA
GSKDTVDVTV
I GTTVAFET P
NDPAGKDQQV
VLIGISFLGG
I DLYDVKNGK
INYTVLKTDG
WDEGSRDKVL
ADKNDPAGKD
KPAKVVVTY.P
EDSIGNLPDL
KVVDPRT DAD V DTAT PG OK.P
NVGETPKAED
ELSI\IOmS\Saro\Kep .pec\639194 doc 261V"91 26 501 GTTVAFETPV V [)PPT DA DKN 551 DPAGKDQQVN
TATPGDKPAK
601 VVVTYPDGSK
GETPKAEDSI
651 GNLPDLPKGT
TVDVTVKVVD
701 PRTDADKNDP
VAFETPVDTA
751 TPGDKPAKVV GK DQQVNVGE 801 TPKAEDSIGN TY PDGS KDT V 851 DVTVKVVDPR P DL PKGTT VA 901 FETPVDTATP
DADKNDPAGK
951 DQQVNVGETP
DKPAKVVVTY
1001 PDGSKDTVDV
AEDSIGNLPD
1051 LPKGTTVAFE
VKVVDPRTDA
1101 DKNDPAGKDQ
PVDTATPGDK
1151 PAKVVVTYPD
VNGKGNKLPA
DTATPGDKPA
VGETPKAEDS
DTV DVTVKVV TVA FET PVDT
AGKDQQVNVG
VTYPDGSKDT
LP DL PKGTT V
TDADKNDPAG
G DKPA KV VVT KA EDSIG NL P
TVK.VVDPRTD
TPVDTATPGD
QVNVGETPKA
GSKDTVDVTV
KVVVTYPDGS
IGNLPDLPKG
DPRTDADKND
AT PGDK PAI V
ETPKAEDSIG
VDVTVKVVDP
A FE-TP VDTAT
KDQQVNVGET
YPDGSKDTVD
DL PKGTT VA F
ADKNDPAGKD
KPAKVVVTY P
EDSIGNLPDL
KVVDPRT DAD
KDTVDVTVKV
TTVAFETPVD
PAGKDQQVNV
VVTYPDGSKD
NLPDLPKGTT
PTDADKNDPA
PG DKPAKVVV P KA EDSIG N L
VTVKVVDPRT
ET P VDTAT PG QQVNVGET PK
DGSKDTVDVT
PKGTTVAFET
KNDPAGKDQQ
1201 TGENATPFFN VVALTIMSSV GLLSVSKKKE D \\MLBOS'meShao n Kee \s secA638 9 i .94.ciot 20/05/91
Claims (14)
1. A purified protein designated Rib, characterized in that: a) it is obtainable from group B streptoococcal strains, especially those of serotype III; b) it is relatively resistant to degradation by trypsin and pepsin; c) it has the N-terminal amino acid sequence according to SEQ ID NO:1 or a sequence at least homologous thereto; and d) it confers protective immunity against group B streptococcal strains expressing the protein; and naturally occurring or artificially modified variants, subfragments and multiples thereof also having ability to confer protective immunity.
2. A protein according to claim 1 wherein the said strain is strain BS30 or BM110 and the protein has an apparent molecular weight of about 95 kD, as determined by SDS PAGE.
3. A protein according to claim 1 or claim 2 having the sequence as set out in SEQ ID NO:4.
4. A process for isolating Rib as defined in Claim 1 or Claim 2, characterised in that a Streptococcus Group B strain expressing the protein is cultivated, the medium and/or the microorganism are isolated, the bacteria are digested with an enzyme, preferably mutanolysin, a protease inhibitor is optionally added, the digested bacteria are separated from the supernant and protein Rib is extracted from the supernant.
5. A process according to claim 4 in which the protein is extracted from the supernatant by dialysis, fractionation by ion-exchange chromatography and gel filtration.
6. An antibody highly specific for protein Rib as defined in any one of claims 1 to 3, or a variant, subfragment or multiple thereof. I 7. A reagent kit for detection of antibodies to \\HELBO1Thonme$\Sharon\xeepspi\6JO91.9 4 .dod 2B/05/97 28 protein Rib, comprising protein Rib or a variant, subfragment or multiple thereof, as defined in claim 1.
8. A reagent kit for detection of protein Rib, comprising an antibody specific to the protein as defined in any one of claims 1 to 3, and optionally protein Rib and/or a variant subfragment and/or multiple thereof as a standard.
9. A vector containing a DNA sequence encoding protein Rib or a variant, subfragment or multiple thereof as defined in anyone of claims 1 to 3. A vector according to claim 9 in which the vector's DNA sequence encoding protein Rib is essentially the same as any of the corresponding DNA sequences of phage lambda Ribl-3,having deposit number DSM 9039. 1% 11. A vector according to claim 9, in which the vector's DNA sequences of phage lambda deposit number DSM 9040.
12. A vector according to claim 9, in which the vector's DNA sequence encoding protein Rib is essentially the same as any of the corresponding DNA sequences of phage lambda Ribl-7, having deposit number DSM 9041.
13. A vector according to claim 9, in which the vector's DNA sequence comprising protein Rib is as set out in SEQ ID NO:3.
14. Phage lambda Ribl-3, having deposit number DSM
9039. Phage lambda Ribl-5, having deposit number DSM
9040. 16. Phage lambda Ribl-7, having deposit number DSM
9041. 17. A DNA sequence encoding protein Rib or a variant, subfragment ormultiple thereof, obtainable from a vector as defined in any one of claims 9 to 13. 18. A DNA sequence encoding protein Rib, as set out in SEQ ID NO:3. 19. A pharmaceutical composition comprising protein Rib or a variant, subfragment or multiple thereof as \\MLBOI\home\Ssharon\1eep\speci\6e99.9 4 doc 28/W,9 29 defined in any one of claims 1 to 7, said composition further comprising a pharmaceutically acceptable adjuvant or excipient. A vaccine comprising protein Rib or variant, subfragment or multiple thereof as defined in any one of claims 1 to 3, said vaccine further comprising a pharmaceutically acceptable adjuvant or excipient. Dated this 2 9 T" day of May 1997 GUNNAR LINDHAL By their Patent Attorneys GRIFFITH HACK Fellows Institute of Patent Attorneys of Australia \\MELBI\home\Sha on\ieep\speci\ 89. 94.doc WOW
Applications Claiming Priority (3)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| WOSE9300234 | 1993-03-19 | ||
| SE9300234 | 1993-03-19 | ||
| PCT/SE1994/000246 WO1994021685A1 (en) | 1993-03-19 | 1994-03-21 | Protein rib, a cell surface protein that confers immunity to many strains of the group b streptococcus; process for purification of the protein, reagent kit and pharmaceutical composition |
Publications (3)
| Publication Number | Publication Date |
|---|---|
| AU6389194A AU6389194A (en) | 1994-10-11 |
| AU681130B2 true AU681130B2 (en) | 1997-08-21 |
| AU681130C AU681130C (en) | 1998-09-24 |
Family
ID=
Also Published As
| Publication number | Publication date |
|---|---|
| ZA941958B (en) | 1995-01-27 |
| KR100331358B1 (en) | 2002-08-13 |
| PT656014E (en) | 2003-09-30 |
| DE69432658D1 (en) | 2003-06-18 |
| ATE240351T1 (en) | 2003-05-15 |
| CA2158658A1 (en) | 1994-09-29 |
| KR960701096A (en) | 1996-02-24 |
| JPH09500092A (en) | 1997-01-07 |
| HUT72841A (en) | 1996-05-28 |
| ES2194024T3 (en) | 2003-11-16 |
| HU217582B (en) | 2000-02-28 |
| SI0656014T1 (en) | 2003-12-31 |
| WO1994021685A1 (en) | 1994-09-29 |
| AU6389194A (en) | 1994-10-11 |
| NZ263275A (en) | 1997-07-27 |
| DE69432658T2 (en) | 2004-04-08 |
| SG47049A1 (en) | 1998-03-20 |
| CN1046291C (en) | 1999-11-10 |
| US5869064A (en) | 1999-02-09 |
| HU9501993D0 (en) | 1995-08-28 |
| DK0656014T3 (en) | 2003-08-11 |
| EP0656014B1 (en) | 2003-05-14 |
| CN1119442A (en) | 1996-03-27 |
| HK1008825A1 (en) | 1999-05-21 |
| EP0656014A1 (en) | 1995-06-07 |
| JP3976334B2 (en) | 2007-09-19 |
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